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Differential Display Technical notes

2024-09-25 DNA 加入收藏
Optimal arbitrary primer length for Differential Display The concept of differen

Optimal arbitrary primer length for Differential Display The concept of differential display is to use a limited number of short arbitrary primers in combination with the anchored oligo-dT primers to systematically amplify and visualize most of the mRNA in a cell. The optimal length of arbitrary primers is determined by statistical consideration that each primer will recognize 50-100 mRNA species. To do so, these primers have to hybridize as 6-8mers (Liang and Pardee, Science. 1992, 257:967.). In practice, however, primers shorter than 9 bases failed to be used for PCR amplification (Williams et al, 1991, Nucleic Acids Res. 18:6531), probably due to the minimum contact surface between Taq polymerase with the double-stranded DNA template. Initially, arbitrary decamers (10mers) were employed for differential display in combination with two-base anchored primers. Although the method worked well in displaying the expected number of mRNA per primer combination under optimal conditions, weak signals, fewer bands, and poorer reproducibility were encountered by people who might have assembled the method under sub-optimal conditions due to the variation in the quality of RNA samples, primers, MMLV reverse transcriptase, isotopes, Taq polymerase and PCR tubes among other things. It is important to point out that the analysis of priming kinetics of arbitrary 10mers under the PCR conditions used has been extremely predictable (Liang and Pardee, 1994, Methods Mol. Gen. 5:3). These primers, as expected, hybridize initially to the first strand cDNA as 6-9mers depending on the GC content, with most of the base-pairing occurred at the 3' end of the primers. To determine the optimal length of arbitrary primers for differential display, we have kept in mind the following essential restrictions:

The theoretical consideration suggests that the optimal selectivity of the arbitrary primers should be provided by no more than 7 bases for each pair of primers to display 50-100 mRNAs. The minimum primer length for PCR is 9 bases. The arbitrary primers have to hybridize in a predictable way in order to rationally design a representative set of such primers to display most of mRNAs in a cell. The arbitrary primers in practice require 8-9 base pair matches for optimal priming. The redundancy (one mRNA species is represented as more than one band in each lane) should be kept to a minimum.

As a result, arbitrary primer length is increased from the sub-optimal value of 9-10 bases to 13 bases. The 13mers fulfill the above criteria for being optimal arbitrary primers (Liang et al., 1994, NAR. 22:5763). First, 13mers are perfect PCR primers as compared to longer primers in terms of being able to specifically amplify a target DNA sequence. They are much more efficient primers than 10mers, producing highly reproducible and uniform band intensities in differential display. Secondly, since the first 6-8 3' bases of these short primers provide the specificity of sequence recognition of the mRNA sequences, the arbitrary 13mers can be rationally designed in such a way that all primers are maximally different in their 7 3' base sequence (bases in bold, see table below), while the 6 5' bases are fixed and statistically can provide an additional 1.5 base pairing for each primer. So the arbitrary 13mers will hybridize as 8-9mers as required in the initial cycle of PCR amplification. Such rational primer design allows a limited number of arbitrary 13mers to be made to ensure that most of the mRNA can be represented (see figure, page 45). PCR conditions used for 10mers were preserved for 13mers to ensure the predictable nature of primer bindings. The table below shows the excellent agreement of the theory for arbitrary primer designs and the actual priming of the arbitrary 13mers in differential display based on the genes cloned.


Other companies have blindly increased the primers to 20 bases or longer in an attempt to increase the "reproducibility" of the cDNA pattern displayed. One has to remember that longer primers are used to amplify specific genes, while shorter primers are used to specifically amplify multiple genes. The longer primers under degenerate conditions will hybridize in a non-predictable way, making a rational design of a representative set of primers impossible. Although, longer primers can also generate a complex cDNA pattern which may appear reproducible, many of the bands may in fact represent the same mRNA due to the "Stickiness" of long primers when used under low stringency. In fact, A. Simpson and colleagues have used this low stringency PCR for long primers to detect sequence polymorphism of the same gene (Simpson et al., 1994, PNAS, 91:1946). To do this, they first specifically amplified a target gene of interest under high stringency conditions. Then, using the DNA sequence specifically amplified as a template and the same pair of long primers to perform PCR under low stringency (decreasing the annealing temperature), they were able to obtain a complex pattern of PCR products from a single template. Therefore the "more reproducible nature" of long primers may be misleading because of the redundancy of the PCR products amplified.


One-base versus two-base anchored primers Recently we asked Dr. Peng Liang about how he came up with the two types of anchored primers used in differential display and which type is better. Here is his explanation: The initial choice of using two-base anchored oligo-dT primers (Liang and Pardee, 1992, Science 257:967; Liang et al., 1993, Nucleic Acids Res. 21:3269.) instead of one-base anchored primers (Liang et al., 1994, Nucleic Acids Res.22:5763.) was due to historical rather than scientific reasons. The initial idea was to use one-base as an anchor, but the cloned murine thymidine kinase (TK) cDNA originally used as a control cDNA template had only 11 A's in its poly(A) tail. It was found that one-based anchored primer T7C up to T11C failed to amplify the TK 3' terminus in combination with an upstream primer specific to TK. Extension of one more base from the 3' end instead of the 5' end of the anchored primer was a logical choice. Interestingly, T11CA started to work successfully in PCR to amplify the expected TK cDNA template. That was how two-base anchored primers were first described. Later, longer one-base anchored primers were shown to be much more efficient for differential display in sub-dividing the mRNA populations into three groups. One-base anchored primers have significant advantages over the two-base anchored primers in that the former reduces the redundancy of priming, eliminates the high background smearing problem for two-base anchored primers ending with the 3' "T", and reduces the number of reverse transcription reactions from 12 to 3 per RNA sample.


Theoretical estimation of the number of arbitrary primers necessary to cover most of the genes expressed in a cell Based on the experimental support that each arbitrary 13mer hybridizes with 7 bases to provide specificity, which represents 1/16,000 possible sequences, a theoretical calculation for the number of arbitrary primers needed to cover most of the expressed genes in a cell can be derived (Liang and Pardee, 1994, Methods Mol. Gen. 5:3). A given mRNA 3' end sequence of 600 bp resolved on a 6% denaturing polyacrylamide gel contains about 600 sites for recognition by all possible 16,000 7mers. Thus each arbitrary primer will have a 600 /16,000 = 4% probability of detecting any given mRNA. This permits an estimation of the number of arbitrary 13mers needed to be rationally designed in order to cover most of 10,000 expressed mRNA species in a mammalian cell. Others have claimed that fewer primers may cover most of the genes expressed, but those calculations were seriously flawed. The number of arbitrary 13mers needed in combinations with all three one-base anchored primers to detect a given fraction of mRNA by differential display.




# Of Arbitrary Primers nReactionsProbability Of Detection P = 1 - (0.96)n



206056%
309071%
4012080%
8024096%



 


Comparison of Differential Display with other methodologies for cloning differentially expressed genes Since its invention in 1992, differential display has quickly overtaken subtractive hybridization to become the method of choice for cloning differentially expressed genes (See Figure below). In fact, since 1992, of the 1800 publications using these 6 techniques, 67% of them have used differential display (1215 out of 1810) based on a Medline search. GenHunter is proud to be the driving force for making differential display accessible to the biomedical research community.


Publications using different methodologies for cloning differentially expressed genes. Subtractive Hybridization, Differential Display, RNA-arbitrarily primed PCR (RAP-PCR), Representational Difference Analysis (RDA), DNA Microarray and Serial Analysis of Gene Expression (SAGE) were compared by Medline search using key words depicting each technology.



Method

Year Invented

Medline entry/yr

Total Entry
Subtractive Hybridization198529404
Differential Display19921741215
RAP-PCR1992426
RDA199323136
DNA Microarray19952183
SAGE1995622

The Medline searches were performed in December, 1999 on OvidWEB using key words depicting the corresponding technologies.


False positives in Differential Display One of the most frequently asked questions for those who want to use differential display is what the false positive rate is. There is really no clear answer to this very complex question, because it depends on so many factors, both intrinsic and extrinsic, of the differential display method. The intrinsic factors include the quality of reagents and enzymes, type and purity of primers, integrity, concentration and purity of RNA used, etc. The extrinsic factors such as the systems being compared, experimental designs, appropriate internal controls, criteria for picking bands, reaction setup, type of PCR reaction tubes, type of thermocyclers, and, of course, the training and experience of a researcher, all can greatly contribute to the rate of false positives. Taking an extrinsic factor, the system being compared, as an example, if one is to compare rat liver versus rat brain where it is known that nearly 50% of the genes expressed are brain specific, the false positives are going to be very low since the difference between samples compared are very large. However, if one is to compare gene expression between the same type of cells with and without a 30 min. treatment of a drug or hormone in hopes of identifying the immediate early genes, the false positives are going to be much higher simply due to the fewer differences in gene expression. Differential display itself can be perfectly reproducible if there are no intrinsic and extrinsic problems. For example, if you set up a 100 mL PCR reaction that is thoroughly mixed and aliquot 20 µL into each of 5 thin-walled PCR reaction tubes, the pattern of cDNA displayed among the five tubes can be perfectly the same. But if instead, 5 individual reactions are set up independently, the cDNA pattern amplified may not be the same simply due to pipetting errors. However, in practice, there is always going to be background "noise" due to pipetting errors because you have to compare different samples. These few spurious bands or "noise" can be as low as 0.1-1% of the cDNA bands displayed, which can be translated to 10-100 bands if you perform all 240 PCR reactions consisting of all the primer combinations in GenHunter's RNAimage® kits. As you can see, given the system that you will be comparing, the false positive rate can be estimated simply as the signal (truly differentially expressed genes) to noise (spurious, non-reproducible bands) ratio. Unlike the comparison between liver and brain, even if you encounter much higher false positives but are able to find the few immediate early genes induced by your drug or hormone, it would be a great accomplishment. The other often-ignored extrinsic factor is the appropriate internal controls. Assuming that you are looking for the immediate early genes induced by a drug or hormone, you must make sure that the treatment truly worked based on either the phenotype of the cells, or more importantly, the induction of a known gene as a control. If this is not done, the differential display comparison is going to be flawed, because there may simply be no difference to begin with if the treatment did not work. In this case, if any differences are found, they are bound to be false positives. For a more detailed review on factors contributing to false positives in differential display, please see Liang and Pardee, 1994. Methods in Mol. Gen. 5:3.; Liang and Pardee, ed., 1997. Differential Display Methods and Protocols, Humana Press (Cat. No.: HP1). There is no doubt that Differential Display is a very dependable method given its enormous popularity and the success of hundreds of thousands of researchers, thanks in part to GenHunter's complete line of reagent systems and step-by-step protocols (see representative publications in the back). Although you can count on GenHunter to solve the intrinsic problems of differential display, having a realistic understanding of the extrinsic problem areas will help you to minimize false positives and eliminate the fears and myths of differential display, one of the most powerful molecular biological tools ever invented.


Frequently used conversion factors


Nucleic Acids

OD260

µg
RNA140
DNA (single-stranded)137
DNA (double-stranded)150


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